AU2008327083A1 - Preparation for application to body surface and preparation holding sheet for application to body surface - Google Patents
Preparation for application to body surface and preparation holding sheet for application to body surface Download PDFInfo
- Publication number
- AU2008327083A1 AU2008327083A1 AU2008327083A AU2008327083A AU2008327083A1 AU 2008327083 A1 AU2008327083 A1 AU 2008327083A1 AU 2008327083 A AU2008327083 A AU 2008327083A AU 2008327083 A AU2008327083 A AU 2008327083A AU 2008327083 A1 AU2008327083 A1 AU 2008327083A1
- Authority
- AU
- Australia
- Prior art keywords
- body surface
- preparation
- target substance
- base
- surface application
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Granted
Links
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- A61K31/70—Carbohydrates; Sugars; Derivatives thereof
- A61K31/7042—Compounds having saccharide radicals and heterocyclic rings
- A61K31/7048—Compounds having saccharide radicals and heterocyclic rings having oxygen as a ring hetero atom, e.g. leucoglucosan, hesperidin, erythromycin, nystatin, digitoxin or digoxin
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/70—Carbohydrates; Sugars; Derivatives thereof
- A61K31/715—Polysaccharides, i.e. having more than five saccharide radicals attached to each other by glycosidic linkages; Derivatives thereof, e.g. ethers, esters
- A61K31/726—Glycosaminoglycans, i.e. mucopolysaccharides
- A61K31/727—Heparin; Heparan
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
- A61K38/16—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- A61K38/17—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- A61K38/19—Cytokines; Lymphokines; Interferons
- A61K38/21—Interferons [IFN]
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- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K47/00—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
- A61K47/30—Macromolecular organic or inorganic compounds, e.g. inorganic polyphosphates
- A61K47/36—Polysaccharides; Derivatives thereof, e.g. gums, starch, alginate, dextrin, hyaluronic acid, chitosan, inulin, agar or pectin
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- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/0012—Galenical forms characterised by the site of application
- A61K9/0019—Injectable compositions; Intramuscular, intravenous, arterial, subcutaneous administration; Compositions to be administered through the skin in an invasive manner
- A61K9/0021—Intradermal administration, e.g. through microneedle arrays, needleless injectors
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/70—Web, sheet or filament bases ; Films; Fibres of the matrix type containing drug
- A61K9/7023—Transdermal patches and similar drug-containing composite devices, e.g. cataplasms
- A61K9/703—Transdermal patches and similar drug-containing composite devices, e.g. cataplasms characterised by shape or structure; Details concerning release liner or backing; Refillable patches; User-activated patches
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61M—DEVICES FOR INTRODUCING MEDIA INTO, OR ONTO, THE BODY; DEVICES FOR TRANSDUCING BODY MEDIA OR FOR TAKING MEDIA FROM THE BODY; DEVICES FOR PRODUCING OR ENDING SLEEP OR STUPOR
- A61M37/00—Other apparatus for introducing media into the body; Percutany, i.e. introducing medicines into the body by diffusion through the skin
- A61M37/0015—Other apparatus for introducing media into the body; Percutany, i.e. introducing medicines into the body by diffusion through the skin by using microneedles
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61M—DEVICES FOR INTRODUCING MEDIA INTO, OR ONTO, THE BODY; DEVICES FOR TRANSDUCING BODY MEDIA OR FOR TAKING MEDIA FROM THE BODY; DEVICES FOR PRODUCING OR ENDING SLEEP OR STUPOR
- A61M37/00—Other apparatus for introducing media into the body; Percutany, i.e. introducing medicines into the body by diffusion through the skin
- A61M37/0015—Other apparatus for introducing media into the body; Percutany, i.e. introducing medicines into the body by diffusion through the skin by using microneedles
- A61M2037/0053—Methods for producing microneedles
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
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Description
1 DESCRIPTION PREPARATION FOR BODY SURFACE APPLICATION AND PREPARATION FOR BODY SURFACE APPLICATION-HOLDING SHEET TECHNICAL FIELD 5 [0001] The present invention relates to a preparation for body surface application and a preparation for body surface application-holding sheet. The preparation for body surface application and the preparation for body surface application-holding sheet according to the present invention can efficiently administer a target substance, and can obtain high absorption 10 rate and high pharmacological effect. BACKGROUND ART [0002] Microneedles (micropiles, micromissile capsules) are under study as a pharmaceutical technology to transdermally administer drugs with high efficiency, where drugs have very low bioavailability and/or low 15 pharmacological availability by a conventional transdermal administration such as painting onto the skin. Microneedles are fine needles that do not give pain even when inserted into the skin. As the materials for microneedles, in addition to the metals used as the conventional injection needles, microneedles made of materials such as silicon have been developed 20 (Non-Patent Documents 1 and 2). These microneedles have the same hollow structure as injection needles, and are used for the injection of drug solution. [0003] Furthermore, self-dissolving type microneedles having biosoluble substance as a base are also developed. Where the target substance is held in the base and is administered into the epiderm followed by the self 25 dissolution of the base when it is inserted into the skin. For example, 2 Patent Documents from 1 to 3 disclose self-dissolving type microneedles made of maltose as a base. Furthermore, Non-Patent Document 1 discloses self-dissolving type microneedles in which a base is made of polycaprolactone, polylactic acid, or polyglycolic acid. Patent Document 4 5 discloses a device or an instrument for injecting a drug via microneedles. [0004] Patent Document 5 discloses microneedles in which a base is made of water-soluble and biosoluble thread-forming polymer. The microneedles increase skin permeability of peptides/proteins such as insulin, erythropoietin and interferon, polysaccharides such as heparin, and vitamin 10 C that are poorly-absorbable through the skin. [0005] Patent Document 6 discloses microneedles in which insoluble particles are localized at an acral side of a microneedle. However, because the acral side becomes brittle with this configuration, it is difficult to maintain physical strength, and there is a possibility to make problems 15 when microneedles are inserted into the skin. [0006] Examples in which microneedles are applied on the body surfaces other than the skin are known. For example, in Non-Patent Document 3, an example in which microneedles are applied onto the cornea is disclosed. [0007] [Patent Document 1] Japanese Patent Laid-Open Publication No. 20 2003-238347 [Patent Document 2] Japanese Patent Laid-Open Publication No. 2005-154321 [Patent Document 31 Japanese Patent Laid-Open Publication No. 2005-152180 25 [Patent Document 4] WO 2004/000389 Pamphlet 3 [Patent Document 5] WO 2006/080508 Pamphlet [Patent Document 6] WO 2007/030477 Pamphlet [Non-Patent Document 1] D. K. Armini and C. Lui, "Microfabrication technology for polycaprolactone, a biodegradable polymer", Journal of 5 Micromechanics and Microengineering, 2000, Vol. 10, pp. 80 to 84 [Non-Patent Document 2] M. R. Prausnitz, Microneedles for transdermal drug delivery, Advanced Drug Delivery Reviews, 2004, Vol. 56, pp. 581 to 587 [Non-Patent Document 3] J. Jiang, Coated Microneedles for Drug 10 Delivery to the Eye, Investigative Ophthalmology & Visual Science, 2007, Vol. 48, pp. 4038 to 4043 DISCLOSURE OF INVENTION PROBLEMS TO BE SOLVED BY THE INVENTION [00081 Based on the technology described in Patent Document 5, protein 15 drugs like erythropoietin can be transdermally administered with high bioavailability. However, protein drugs such as erythropoietin and interferon are very expensive. Therefore, there is a need for a technology that has higher administration efficiency and make possible the higher bioavailability and pharmacological availability. The situation is the same 20 in the case of the administration of a drug via body surfaces other than the skin. [0009] It is an objective of the present invention to provide self-dissolving microneedles that can realize higher absorption efficiency and higher pharmacological effect. 25 MEANS FOR SOLVING THE PROBLEMS 4 [00101 In the process of performing further research on microneedles, the present inventor has discovered a new problem. Specifically, in the conventional self-dissolving type microneedle, a target substance is uniformly held in the whole base. Further, from the point of ease of 5 handling (for example, ease of insertion into the skin), it is preferred to use microneedles having a total length of about 500 micrometers (for example, see James C. Birchall, "Chapter 18: Stratum corneum bypassed or removed" in Enhancement in Drug Delivery, ed. By Elka Touitou and Brian W. Barry, pp. 337-351, 2007, CRC Press.). However, the present inventor has 10 discovered the phenomenon that when a microneedle with this size is inserted into the skin by pressing with a finger, total length of microneedles may not be inserted into the skin, and part of the rear end portion remains out of the skin. Consequently, in practice the target substance which is present in the rear end portion is discarded without being absorbed into the 15 skin. The present inventor has found that this loss is an obstacle to improving bioavailability and pharmacological availability. In particular, in case that the target substance is an expensive protein drug, even if the loss is small, this is a large problem when commercializing the product. Accordingly, the present inventor continued research to solve this problem, 20 and completed the below-described invention. [0011] One aspect of the present invention is a needle-shaped preparation for body surface application, comprising a base formed from a biosoluble substance and a target substance held in the base, the preparation for body surface application being used by being inserted into a body surface, and the 25 target substance being absorbed into the body by dissolution of the base, 5 wherein the preparation for body surface application is formed of two or more sections divided in the insertion direction; the target substance is held in at least one section other than the rearmost end section; and the section in which the target substance is held is obtained by solidifying the base in 5 which the target substance is dissolved. [0012] The preparation for body surface application according to this aspect has a needle shape, is used by being insertied into a body surface such as the skin, the target substance is absorbed into the body by dissolution of the base. The section in which the target substance is held is 10 composed of the "stuff obtained by solidifying the base in which the target substance is dissolved" (hereinafter, the target substance is sometimes referred to as the "target substance soluble in base"). Furthermore, the preparation for body surface application according to the present invention is formed of two or more sections divided in the insertion direction. The 15 target substance is held in at least one section other than the rearmost end section. Therefore, when the preparation for body surface application according to this aspect is inserted into the skin and the like, even if the rearmost end section remains out of the body surface, loss of the target substance can be kept to the minimum. Consequently, higher absorption 20 efficiency and higher pharmacological effect of the target substance can be realized. [0013] Here, the "body surface" means a surface portion of the body which is in contact with the outside. In the present invention, the body surface includes skin, cornea, oral soft tissue, gum, nasal cavity mucosa membrane 25 and the like. Furthermore, the "preparation for body surface application" 6 means a preparation which can be inserted into, closely adhered to, or pasted on a body surface to administer a target substance into the body. A representative example of the preparation for body surface application is a transdermally absorbable preparation. Obviously, preparations which are 5 used by inserting into, closely adhering to, or pasting on the cornea or the oral cavity mucosa are also included in the preparation for body surface application according to the present invention. [0014] Another aspect of the present invention is a needle-shaped preparation for body surface application, comprising a base formed from a 10 biosoluble substance and a target substance held in the base, the preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the preparation for body surface application is formed of two or more sections divided in the insertion direction; the 15 target substance is held in at least one section other than the rearmost end section; and the section in which the target substance is held is obtained by solidifying (a) the base in which cells are dispersed, (b) the base in which the target substance is dispersed as a lipid dispersion, or (c) the base in which the target substance formed from fine particles having an average particle 20 size of 10 micrometers or less is dispersed. [00151 For the preparation for body surface application according to this aspect too, when inserted into a body surface, even if the rearmost end section remains out of the body surface, loss of the target substance can be kept to the minimum. Consequently, higher absorption efficiency and 25 higher pharmacological effect of the target substance can be realized.
7 Furthermore, for the preparation for body surface application according to this aspect, the section in which the target substance is held is formed from the "stuff obtained by solidifying the base in which the target substance is dispersed" (hereinafter, the target substance is sometimes referred to as the 5 "target substance dispersible in base"), and the target substance is any of the above-described (a) to (c). Therefore, physical strength of the preparation is maintained, and insertion into the body surface is easy. [00161 Preferably, the target substance is held in the frontmost end section. 10 [00171 According to this preferable aspect, the section containing the target substance is reliably inserted into the skin and the like. [00181 Preferably, the total length in the insertion direction is in a range of 200 to 600 micrometers. [0019] Preferably, the total length in the insertion direction is in a range 15 of 400 to 600 micrometers. [0020] According to this preferable aspect, especially, when inserting into the skin and the like by pressing with a finger, the section containing the target substance is reliably inserted into the skin and the like. [0021] A sum of the lengths in the insertion direction of the sections 20 excluding the rearmost end section is 350 micrometers or less. [0022] According to this preferable aspect, the section containing the target substance is reliably inserted into the skin and the like. [00231 Another aspect of the present invention is a needle-shaped preparation for body surface application, comprising a base formed from a 25 biosoluble substance and a target substance held in the base, the 8 preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the target substance is not uniformly distributed in the base along the insertion direction with more of the target 5 substance present towards a tip side than a rear end side; and the portion in which the target substance is present is obtained by solidifying the base in which the target substance is dissolved. [00241 The preparation for body surface application according to this aspect also has a needle shape, is used by being inserted into a body surface 10 such as the skin, and the target substance is absorbed into the body by dissolution of the base. The section in which the target substance is held is formed from the "stuff obtained by solidifying the base in which the target substance is dissolved". In other words, the target substance is soluble in base. Furthermore, in the preparation for body surface application 15 according to the present invention, the target substance is not uniformly distributed in the base along the insertion direction with more of the target substance present towards a tip side than a rear end side. Therefore, when the preparation for body surface application according to this aspect is inserted into the skin and the like, even if the rear end portion of the 20 preparation remains out of the body surface, loss of the target substance can be kept to the minimum. Consequently, higher absorption efficiency and higher pharmacological effect of the target substance can be realized. [0025] Another aspect of the present invention is a needle-shaped preparation for body surface application, comprising a base formed from a 25 biosoluble substance and a target substance held in the base, the 9 preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the target substance is not uniformly distributed in the base along the insertion direction with more of the target 5 substance present towards a tip side than a rear end side; and the portion in which the target substance is present is obtained by solidifying (a) the base in which cells are dispersed, (b) the base in which the target substance is dispersed as a lipid dispersion, or (c) the base in which the target substance formed from fine particles having an average particle size of 10 micrometers 10 or less is dispersed. [0026] For the preparation for body surface application according to this aspect too, when inserted into a body surface, even if the rearmost end section remains out of the body surface, loss of the target substance can be kept to the minimum. Consequently, higher absorption efficiency and 15 higher pharmacological effect of the target substance can be realized. Furthermore, for the preparation for body surface application according to this aspect, the target substance soluble in base is any of the above described (a) to (c). Therefore, physical strength of the preparation is maintained, and insertion into the body surface is easy. 20 [0027] Preferably, the total length in the insertion direction is in a range of 200 to 600 micrometers. [00281 Preferably, the total length in the insertion direction is in a range of 400 to 600 micrometers. [0029] Preferably, the target substance is held in a portion within 350 25 micrometers from the tip towards the rear end.
10 [00301 Another aspect of the present invention is a needle-shaped preparation for body surface application, comprising a base formed from a biosoluble substance and a target substance held in the base, the preparation for body surface application being used by being inserted into a 5 body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the preparation for body surface application is formed of three or more sections divided in the insertion direction; the target substance is held in at least one section which is not either the frontmost end section or the rearmost end section; and the section in which 10 the target substance is held is obtained by solidifying the base in which the target substance is dispersed. [00311 The preparation for body surface application according to this aspect is formed of three or more sections divided in the insertion direction. The target substance (dispersible in base) is held in at least one section 15 which is not either the frontmost end section or the rearmost end section. Therefore, when the preparation for body surface application according to this aspect is inserted into the skin and the like, even if the preparation rear end portion remains out of the body surface, loss of the target substance can be kept to the minimum. Consequently, higher absorption efficiency and 20 higher pharmacological effect of the target substance can be realized. In addition, since the target substance is held in a section positioned nearer (rear end side) than the frontmost section, when applying to the skin for example, more of the target substance can be delivered to a closer portion in the epidermis of the skin. Still further, since the target substance 25 (dispersible in base) is not held in the frontmost section, physical strength of 11 the frontmost section is maintained, and insertion into the body surface is easy. [0032] Preferably, the target substance is held in a section adjacent to the frontmost end section. 5 [0033] According to this preferable aspect, when applying to the skin for example, more of the target substance can be delivered to a closer portion in the epidermis of the skin. [0034] Preferably, the total length in the insertion direction is in a range of 200 to 600 micrometers. 10 [0035] Preferably, the total length of the preparation in the insertion direction is in a range of 400 to 600 micrometers. [0036] Preferably, a sum of the lengths in the insertion direction of the sections excluding the rearmost end section is 350 micrometers or less. [0037] Preferably, the target substance comprises (i) one encapsulated in a 15 microcapsule or (ii) fine particles having an average particle size of 10 micrometers or less. [00381 Preferably, the body surface comprises skin, cornea, oral soft tissue, gum, or nasal cavity mucous membrane. [00391 Preferably, the base is a high molecular weight substance. 20 [00401 Preferably, the high molecular weight substance is at least one kind selected from the group consisting of polysaccharides, proteins, polyvinyl alcohols, carboxy vinyl polymers, cop olymers of these substances, and salts of these substances. [00411 Preferably, the target substance is peptides, proteins, nucleic acids, 25 or polysaccharides.
12 [0042] Preferably, the target substance is drugs, vaccines, nutrients, or components for cosmetics. [00431 Preferably, the base includes a porous substance, and the target substance is held in the porous substance, so that the target substance is 5 sustainedly released. [00441 Yet another aspect of the present invention is a preparation for body surface application-holding sheet, in which one or two or more of the preparation for body surface application according to the present invention are held on at least one surface of a sheet-like support, wherein the 10 preparation for body surface application can be inserted into a body surface by pressing against the body surface. [0045] The preparation for body surface application-holding sheet according to this aspect comprises the preparation for body surface application according to the present invention. According to this aspect, the 15 preparation for body surface application of the present invention can be easily and efficiently administered. [00461 Preferably, the preparation for body surface application includes an adhesive substance in the rearmost end section. [0047] According to this preferable aspect, the preparation for body 20 surface application is reliably held by the support. ADVANTAGES OF THE INVENTION [0048] According to the preparation for body surface application of the present invention, a target substance can be administered via a body surface with higher absorption efficiency and higher pharmacological effect. 25 Consequently, the preparation for body surface application of the present 13 invention is especially useful when the target substance is expensive. [0049] Similarly, for the preparation for body surface application-holding sheet according to the present invention, a target substance can be administered via a body surface with higher absorption efficiency and 5 higher pharmacological effect. Furthermore, the preparation for body surface application according to the present invention can be easily and efficiently administered. BRIEF DESCRIPTION OF THE DRAWINGS [0050] 10 Fig. 1 is a perspective view illustrating a preparation for body surface application according to a first embodiment of the present invention. Fig. 2 is a front view of the preparation for body surface application of Fig. 1. Fig. 3 is a cross-sectional view illustrating a state in which the preparation for body surface application of Fig. 1 is inserted into the skin. 15 Fig. 4 is a front view illustrating a modified example of the preparation for body surface application of Fig. 1. Fig. 5 is a perspective view illustrating a preparation for body surface application according to a second embodiment of the present invention. Fig. 6 is a front view of the preparation for body surface application of Fig. 5. 20 Fig. 7 is a front view illustrating a modified example of the preparation for body surface application of Fig. 5. Fig. 8(a) is a perspective view illustrating a preparation for body surface application according to another embodiment of the present invention, and Fig. 8(b) is a perspective view illustrating a preparation for body surface 25 application according to yet another embodiment of the present invention.
14 Fig. 9 is a perspective view illustrating a preparation for body surface application-holding sheet according to an embodiment of the present invention. Fig. 10 is a photograph of the microneedle array produced in Example 5. 5 Fig. 11 is a graph showing the temporal transitions of the blood glucose level after the microneedles produced in Examples 5 and 6 were administered to a rat. Fig. 12 is a graph showing the temporal transitions of serum EPO level after the microneedles produced in Examples 7 and 8 were administered to a rat. 10 Fig. 13 is a graph showing the temporal transitions of plasma desmopressin level after the microneedles produced in Example 14 were administered to a rat, and temporal transitions after intravenous injection. Fig. 14 is a photograph of the microneedle array produced in Example 16. Fig. 15 is a photograph of the microneedle array produced in Example 25. 15 Fig. 16 is a graph showing the temporal transitions of serum EPO level after the microneedles produced in Example 29 were administered to a rat. DESCRIPTION OF THE REFERENCE NUMERALS [00511 1, la to li ... Preparation for body surface application, 20 2 ... Body surface insertion end (tip), 3 ... Pressing end (rear end), 5 ... Tip portion (section), 6, 6a to 6i ... Rear end portion (section), 7, 7a to 7c ... Middle portion (section), 25 8 ... Skin (body surface), 15 21, 22, 23, 25, 26 ... Preparation for body surface application, 50 ... Preparation for body surface application-holding sheet, 58 ... Support. BEST EMBODIMENT FOR CARRYING OUT THE INVENTION 5 [00521 A best embodiment for carrying out the invention will now be described. As illustrated in Figs. 1 and 2, a preparation 1 for body surface application according to a first embodiment of the present invention is a solid preparation which is generally called microneedles, micropiles, micromissile capsules and the like. This preparation 1 for body surface 10 application has a needle shape, specifically, a cone shape. The preparation 1 for body surface application has a body surface insertion end 2 with a tapered shape at the frontmost end thereof, and a pressing end 3 at the rearmost end formed in a roughly circular flat surface. The preparation 1 for body surface application is used by being inserted into the body surface 15 such as the skin by pressing the pressing end 3 in a state in which the body surface insertion end 2 is in contact with the body surface. [00531 The preparation 1 for body surface application has a total length H of approximately 500 micrometers (pm). The pressing end 3 has a diameter D of approximately 300 pm. The possible ranges for the total length H of 20 the preparation 1 for body surface application and the diameter D of the pressing end 3 thereof are not especially limited, as long as the values allow the preparation 1 for body surface application to be used as microneedles. For example, H has a value which may be selected from the range of 50 to 1,500 pm, preferably 100 to 1,000 sm, more preferably 200 to 600 jim, and 25 still more preferably 400 to 600 pm. In particular, when the preparation is 16 inserted into the body surface by pressing with a finger, a range of 400 to 600 gm is easy to use. Furthermore, D has a value which may be selected from the range of, for example, 50 to 500 pm, preferably 100 to 450 gm, and more preferably 200 to 400 pm. From the perspective of strength, D is 5 preferably 1/2 of H to the same value as H, and more preferably 2/3 of H to the same value as H. [00541 In the preparation 1 for body surface application, the target substance is not uniformly distributed (localized) in the base along the insertion direction, and the content density of the target substance at the 10 side of the body surface insertion end 2 is larger than the content density of the target substance at the side of the pressing end 3. Specifically, the preparation 1 for body surface application has two sections divided in the insertion direction, namely, a tip portion 5 and a rear end portion 6. The tip portion 5 is a section including the body surface insertion end 2, and is 15 formed from the base which holds the target substance. More specifically, the tip portion 5 is formed from the "stuff obtained by solidifying the base in which the target substance is dissolved". In other words, the target substance is soluble in base. Consequently, the target substance is present in the base as a solid dispersion or a supramolecular complex. On the other 20 hand, the rear end portion 6 is a section including the pressing end 3, and is formed mainly only from the base. The rear end portion 6 does not hold the target substance. The boundary between the tip portion 5 and the rear end portion 6 is a roughly flat surface. Specifically, while in the conventional self-dissolving type microneedles the target substance is uniformly held in 25 the base, in the preparation 1 for body surface application of the present 17 embodiment, the target substance is held non-uniformly with a bias in the base. The base is made from biosoluble substances. [00551 The tip portion 5 has a length L in the insertion direction of approximately 300 gim. The possible range for L may be appropriately 5 selected based on the insertable depth into the body surface. For example, when the preparation is inserted into the body surface by pressing with a finger, L is preferably 350 pm or less, and more preferably 300 sm or less. While the lower limit is not especially limited, it may be, for example, 100 pm or more. Concerning the pressure when inserting the microneedle into 10 the skin by hand (manual insertion into the skin), there is a disclosure of 0.35 to 0.5 N (Kolli et al., Pharmaceutical Research, Vol. 25, pp. 104 to 113 (2007)). [00561 Fig. 3 illustrates a state in which the preparation 1 for body surface application is inserted into skin (body surface) 8 by pressing with a finger. 15 When the preparation 1 for body surface application is inserted into the skin 8 by pressing with a finger, usually only about 300 to 350 gm of the tip side is inserted into the skin 8. About 150 to 200 pIm of the rear end side remains outside the skin 8. However, in the preparation 1 for body surface application, the target substance is contained in the tip portion 5. Therefore, 20 as shown in Fig. 3, even if part or all of the rear end portion 6 is not inserted into the skin 8 and remains outside of the skin 8, high absorption efficiency and high pharmacological effect can be realized where the actual dose of the target substance does not decrease below its desired dose. Furthermore, since the target substance is not contained in the rear end portion 6, the 25 target substance is not wasted, so that economical effect is high. Therefore, 18 from a practical standpoint, the effects are very high. [0057] In the present embodiment, the target substance held in the tip portion 5 is soluble in base. However, the target substance may also be used in the tip portion 5 even if it is dispersible in base. Specifically, the stuff 5 obtained by solidifying (a) the base in which cells are dispersed, (b) the base in which a target substance is dispersed as lipid dispersion, or (c) the base in which a target substance formed from fine particles having an average particle size of 10 micrometers or less is dispersed, may be used. If the target substance is dispersible in base like (a) to (c), problems do not 10 especially occur during insertion into the body surface since physical strength of the tip portion 5 is maintained. [00581 Examples of the cell of (a) include red blood cells. Further, examples of the lipid dispersion of (b) include liposome preparations, emulsions and the like. In addition, while the fine particles of (c) preferably 15 have an average particle size of 10 micrometers or less, more preferred is 5 pm or less, and even more preferred is 2 jim or less. More specifically, if the average particle size is more than 10 pm, the section becomes brittle, which makes it difficult to maintain physical strength of the tip portion 5. Consequently, the tip portion 5 is crushed during insertion into the skin and 20 the like, so that insertion becomes difficult. [0059] In the present embodiment, although the rear end portion 6 is formed only from biosoluble base, an adhesive substance may optionally be formulated. [0060] Although the method for producing the preparation 1 for body 25 surface application is not especially limited, a method which uses a mold 19 may be used, for example. First, a mold having cone-shaped pores is prepared. Then, a substance for forming the base is dissolved with a solvent, and a target substance is further dissolved or dispersed therein to prepare a liquid base that contains the target substance. This liquid base containing 5 target substance is charged into the cone-shaped mold, whereby a tip portion 5 is formed. At this stage, it is preferred to perform centrifugation or to apply pressure so that the liquid base reaches right into the depths of the mold. Next, a liquid base which does not contain the target substance is prepared and further charged into the mold so as to be superimposed over 10 the target substance-containing base. Consequently, a rear end portion 6 is formed. Then, the bases are solidified, and a cone-shaped solid stuff is removed from the mold. The produced solid stuff is formed as the needle shaped preparation 1 for body surface application having two sections (tip portion 5 and rear end portion 6) as illustrated in Figs. 1 and 2. 15 [0061] In the preparation 1 for body surface application, the length L in the insertion direction of the tip portion 5 is approximately 300 gm. However, this length L may be even shorter. Although a preparation for body surface application 21 shown in Fig. 4 has the same external form as the preparation 1 for body surface application shown in Figs. 1 and 2, the 20 length L of the acral portion 5 is approximately 100 im. The target substance is concentrated in the portion near the body surface insertion end 2. [0062] The preparations for body surface application 1 and 21 are both divided into two or more sections. However, the present invention is not 25 limited to these embodiments. Specifically, as long as the target substance 20 is not uniformly distributed (localized) in the base along the insertion direction, and the content density of the target substance at the side of the body surface insertion end 2 is larger than the content density of the target substance at the side of the pressing end 3, the portion containing the target 5 substance and the other portions do not have to be divided with a clear interface. For example, the content density of the target substance may gradually increase from the pressing end 3 towards the body surface insertion end 2, so that the density change is continuous. [0063] A preparation 22 for body surface application according to a second 10 embodiment illustrated in Figs. 5 and 6 has three sections divided in the insertion direction. More specifically, a middle portion 7 is arranged between the tip portion 5 including the body surface insertion end 2 and the rear end portion 6 including the pressing end 3. The target substance is held in the middle portion 7. The middle portion 7 is formed from the "stuff 15 obtained by solidifying the base in which the target substance is dispersed". In other words, the target substance held in the middle portion 7 is dispersible in base. On the other hand, the tip portion 5 and the rear end portion 6 are both sections formed mainly only from a base. These portions do not hold the target substance. The length of the portions in the 20 preparation 22 for body surface application excluding the rear end portion 6, namely, a sum length Li of the tip portion 5 and the middle portion 7, is approximately 300 gm, which is about the same as the length of the acral portion 5 of the preparation 1 for body surface application illustrated in Figs. 1 and 2. Therefore, if the preparation 22 for body surface application is 25 inserted into the body surface such as the skin by pressing with a finger, 21 usually all of the middle portion 7 will enter the body surface. Consequently, high absorption efficiency and high pharmacological effect of the target substance can be realized. In addition, when applying to the skin for example, more of the target substance can be delivered to the epidermis 5 than to the dermis. Still further, since the target substance dispersible in base is not held in the tip portion 5, physical strength of the tip portion 5 is high. Consequently, insertion of the preparation 22 for body surface application into the body surface is easy. The preparation 22 for body surface application can be obtained by, for example, superimposing in order 10 the liquid bases corresponding to the tip portion 5, the middle portion 7, and the rear end portion 6 on the above-described cone-shaped mold, and solidifying the liquid bases. [0064] Representative examples of the target substance dispersible in base held in the middle portion 7 include a target substance formed from the 15 microp articles insoluble in base. Examples of such a target substance include G) a target substance encapsulated in a microcapsule; and (ii) a target substance of microparticles having an average particle size of 10 pm or less. [0065] When using a target substance soluble in base or a target 20 substance dispersible in base as described in the (a) to (c), the target substance may be held in the tip portion 5, or may be held in both the middle portion 7 and the tip portion 5. Furthermore, different target substances may be held in the middle portion 7 and the tip portion 5, respectively. For example, a target substance dispersible in base may be 25 held in the middle portion 7 and a target substance soluble in base may be 22 held in the tip portion 5. [0066] The middle portion may be formed of a plurality of sections. The preparation 23 for body surface application illustrated in Fig. 7 has five sections divided in the insertion direction, namely, a tip portion 5, middle 5 portions 7a, 7b, and 7c, and a rear end portion 6. Specifically, the preparation 22 for body surface application has three middle portions 7a, 7b, and 7c between the tip portion 5 and the rear end portion 6. The middle portions 7a, 7b, and 7c are layered in that order. The middle portion 7a is in contact with the rear end portion 6, and the middle portion 7c is in contact 10 with the tip portion 5. The length of the portions in the preparation 23 for body surface application excluding the rear end portion 6, namely, a sum length L2 of the acral portion 5 and the middle portions 7a, 7b, and 7c, is approximately 300 micrometers, which is about the same as the length of the acral portion 5 of the preparation 1 for body surface application 15 illustrated in Figs. 1 and 2. -According to the preparation 23 for body surface application, for example, different target substances dispersible in base may be held in the middle portions 7a, 7b, and 7c, respectively. Obviously, a target substance soluble in base or a target substance dispersible in base as described in the (a) to (c) may also be held in the tip portion 5. 20 [00671 In the above-described embodiments, although the rear end portion 6 does not contain the target substance, the present invention is not limited to this. For example, the present invention also includes an aspect in which a small amount of a target substance is unintentionally contained in the rear end portion 6. 25 [0068] In the above-described embodiments, while all of the preparations 23 for body surface application had a cone-shaped external form, the present invention is not limited to this shape. As long as the preparation for body surface application is "needle-shaped", another shape may be employed. Specifically, any shape generally considered to be a microneedle, micropile, 5 micromissile capsule shape or the like is included in the present invention. For example, the four-sided pyramid-shaped preparation 25 for body surface application illustrated in Fig. 8(a), and the nail-shaped preparation 26 for body surface application illustrated in Fig. 8(b) are included in the needle shaped preparation for body surface application according to the present 10 invention. In addition, all of the shapes of the transdermal absorption preparation described in WO 2006/080508 pamphlet are also included in the "needle shaped". Furthermore, a neck or a cleavage line may also be provided on the surface of the preparation for body surface application according to the present invention. 15 [0069] Next, an embodiment of a preparation for body surface application holding sheet according to the present invention will be described. A preparation for body surface application-holding sheet 50 shown in Fig. 9 is a patch made of a sheet-like support 58 and nine preparations la to li for body surface application. The preparations la to 1i for body surface 20 application are held on one surface of the support 58. Furthermore, the preparations la to li for body surface application can be inserted by pressing the preparation for body surface application-holding sheet 50 into a body surface such as the skin. The preparation for body surface application holding sheet 50 is also called as the "microneedle array". The preparations 25 la to ii for body surface application have the same basic structure as the 24 preparation 1 for body surface application illustrated in Figs. 1 and 2. However, the preparations la to li for body surface application contain an adhesive substance in respective rear end portions 6a to 6i. Consequently, the preparations la to 1i for body surface application can be reliably held on 5 the support 58 via the rear end portions 6a to 6i. Examples of adhesive substances which can be used include substances and materials employed for the adhesive tape of pharmaceuticals, such as acrylic acids, acrylates, copolymers thereof, and silicone-based adhesives and the like. It is preferred that the support 58 is formed from a material which has a stable 10 strength. However, the support 58 may also be formed from a flexible material. For example, a paper board or various kinds of medical tape such as a cloth adhesive bandage can be employed as the support 58. Further, after pressing the preparation for body surface application-holding sheet 50 against the body surface, the support 68 may be pasted on the body surface 15 as it is, or only the support 58 may be peeled off and removed. In the former case, an adhesive substance may be coated on the whole pasting surface of the support 58 so that the support 58 is reliably pasted on the body surface. [00701 Next, the base and the target substance will be described. The base used in the preparation for body surface application according to the present 20 invention is formed from a biosoluble substance. This substance may be a high molecular weight substance or a low molecular weight substance (for example, maltose). [00711 In a preferred embodiment, the base is formed from a high molecular weight substance. In a more preferred embodiment, the high 25 molecular weight substance is at least one kind selected from the group 25 consisting of polysaccharides, proteins, polyvinyl alcohols, carboxy vinyl polymers, copolymers of these substances, and salts of these substances. One kind of such high molecular weight substances may be used, or the combination of a plurality of kinds may be used. Further, polysaccharides, 5 proteins, polyvinyl alcohols, and carboxy vinyl polymers are all the high molecular weight substances which are water soluble and thread-formable. [0072] Examples of polysaccharides include hyaluronic acid, chondroitin sulfate, dextran, dextran sulfate, alginic acid, glycogen, hydroxypropyl cellulose, hydroxypropyl methylcellulose phthalate, agarose, chitin, chitosan, 10 pectin, and pullulan, and salts thereof. One kind of such a polysaccharide may be used, or the combination of a plurality of kinds may be used. Examples of the protein include serum albumin, serum a acidic glycoprotein, gelatin, and salts thereof. One kind of such a protein may be used, or a combination of a plurality of kinds may be used. Obviously, the 15 polysaccharide and the protein may be used in combination. [0073] On the other hand, the target substance is not especially limited. Any substance may be used as the target substance, for example a high molecular weight substance, a low molecular weight substance, a chemical substance, a physiologically active substance, proteins (recombinant or 20 natural), peptides, polysaccharides and the like. Preferred examples include peptides, proteins, nucleic acids, or polysaccharides. As described above, cells may also be used as the target substance. Furthermore, as the application, a configuration in which the target substance comprises drugs, vaccines, nutrients, or components for cosmetics is also preferred. If the 25 target substance is a drug or a vaccine (a vaccine antigen), the preparation 26 for body surface application of the present invention can be used in the treatment, prevention, diagnosis and the like of a disease. Furthermore, if the target substance is a component for cosmetics, the preparation for body surface application of the present invention can be used for purposes of 5 prevention and improvement of skin aging, anti-aging, skin whitening maintenance, and the like. Examples of the nutrients include health foods and functional food components. Although specific examples of substances which can be employed as the target substance in the preparation for body surface application according to the present invention will now be described 10 below, the target substance of the present invention is not limited to these. [00741 [Examples of Transdermally Poorly- or Low-absorbable High Molecular Weight Substances] Examples include: insulin; interferon; erythropoietin (EPO); tumor necrosis factor (TNF); granulocyte colony-stimulating factor (G-CSF); granulocyte 15 monocyte colony-stimulating factor (GM-CSF); calcitonin; chorionic gonadotropin; desmopressin acetate; growth hormone; vaccines such as influenza vaccine, hepatitis vaccine, and polio vaccine; leuprorelin acetate; Botulinum toxin; glucocerebrosidase; factor VII; ovary-stimulating hormone; ghrelin; various growth factors such as platelet-derived growth factor 20 (PDGF); and nucleic acids such as DNA, RNA, oligo nucleotides (for example, for antisense). [00751 [Examples of Transdermally Poorly- or Low-absorbable Drugs] Examples include diclofenac and the like. [Examples of Drugs for Corneal Administration] 25 Examples include pilocarpine hydrochloride and the like.
27 [Examples of Drugs for Oral Cavity Mucosal Membrane Administration] Examples include lidocaine hydrochloride and the like. [Examples of Nutrients] Examples include vitamin C (ascorbic acid) and the like. 5 [Examples of a Component for a Cosmetic] Examples include retinol and the like. [0076] The preparation for body surface application according to the present invention can be used as a sustained-release preparation. In one embodiment, the base includes a porous substance. The target substance is 10 held in the porous substance, and is sustainedly released. Examples of the porous substance include silicates such as calcium silicate, aluminum silicate, and magnesium silicate; anhydrous silicic acid; porous carbonates such as porous calcium carbonate; porous phosphates such as porous calcium phosphate; porous silicon and the like. One kind of such a porous 15 substance may be used, or a combination of a plurality of kinds may be used. [0077] In another embodiment, the target substance is a long-acting type substance, and the target substance is sustainedly released. Examples of long-acting type substances include long-acting insulin, and polyethylene glycol (PEG)-crosslinked proteins. Specific examples of long-acting insulin 20 include intermediate-, long-, and super long-acting insulins. Specific examples of PEG-crosslinked proteins include PEG-modified proteins such as PEG-interferon and PEG-erythropoetin. [0078] According to the present invention, a method for administering a target substance is provided, in which a needle-shaped preparation for body 25 surface application is inserted into a body surface so that the target 28 substance is absorbed into the body. Similarly, a method for administering a target substance is provided in which a preparation for body surface application-holding sheet is attached on a body surface so that the target substance is absorbed into the body. 5 [0079] The present invention will now be described in more detail based on the following examples. However, the present invention is not limited to these examples. Example 1 [00801 One hundred (10 lines x 10 columns) inverted cone-shaped pores 10 having a depth of approximately 500 micrometers (gm) and a basement diameter of approximately 300 micrometers were arranged on a surface of a substrate made of a silicon resin which was a square with a bottom face 1 cm long and 1 cm wide. This substrate was used as the mold for production of microneedle (preparation for body surface application) or 15 patch/microneedle array (preparation for body surface application-holding sheet). This mold was used in the present example as well as in the subsequent examples. [00811 A viscous dense solution (solution Al) was prepared by adding 80 microliters (pL) of purified water to 30 mg of insulin sodium salt (self 20 prepared product; target substance), 0.2 mg of evans blue (Nacalai Tesque, Inc.), and 30 mg of chondroitin sulfate C sodium salt (Wako Pure Chemical Industries, Ltd.; base), and thoroughly dissolving and mixing the resultant mixture. Furthermore, a dense solution (solution BI) was prepared by adding 30 pL of purified water to 30 mg of chondroitin sulfate C sodium salt 25 and 0.5 mg of Hiviswako 103 (Wako Pure Chemical Industries, Ltd.; 29 adhesive substance), and thoroughly dissolving and mixing the resultant mixture. In addition, an adhesive (solution C1) was prepared by adding 36 mL of purified water to 1.6 g of Hiviswako 103, and thoroughly dissolving and mixing the resultant mixture. 5 [0082] Solution Al was coated and filled into each of the mold pores, and the surface was then covered with a wrapping film (Saran Wrap*; Asahi Kasei Corporation). The mold was set in a table-top centrifuge (Kubota 4000), and centrifuged for 5 minutes at 3,000 rpm. Consequently, the solution Al was filled into the pores more towards the deeper end (tip side) 10 of the pores, so that a space was formed at the near side (rear end side) of the pores. [00831 The wrapping film was taken off, and residue on the mold surface was removed. Next, the solution B1 was coated and filled into each of the mold pores, and the surface was then covered with a wrapping film. The 15 mold was set in a table-top centrifuge, and centrifuged for 5 minutes at 3,000 rpm. Consequently, the solution B1 was filled into the pores, and superimposed over the solution Al. The solution C1 was coated on a paper sheet (support), then covered and pasted onto the whole surface of the mold. The mold was centrifuged for 5 minutes at 3,000 rpm by a table-top 20 centrifuge to dry and solidify each of the viscous solutions in the mold. The paper sheet was slowly peeled off, so that the needle-shaped solid stuff (microneedles) was removed from the mold while still held on the paper sheet. Consequently, a patch/microneedle array (preparation for body surface application-holding sheet) holding 100 microneedles (preparations 25 for body surface application) was obtained. Any of the 100 microneedles 30 held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing the insulin sodium salt and a rear end portion containing the adhesive substance. The tip portions were colored blue due to the presence of the evans blue. 5 Example 2 [00841 A dense solution was prepared by adding 80 sL of purified water to 30 mg of chondroitin sulfate C sodium salt (Wako Pure Chemical Industries, Ltd.; base). A viscous, dense suspension (solution A2) was prepared by adding to this dense solution 30 mg of diclofenac sodium salt (Wako Pure 10 Chemical Industries, Ltd.; target substance) produced to have a particle size of about 5.0 gm by pulverizing it with a mortar made from agate, and mixing the resultant mixture. Furthermore, an adhesive solution (solution B2) was prepared by adding 35 mL of purified water to 1.6 g of Hiviswako 103, and dissolving the resultant mixture. In addition, a dense solution 15 (solution C2) was prepared by adding 0.8 mL of purified water to 300 mg of chondroitin sulfate C sodium salt, and thoroughly dissolving the resultant mixture. [00851 In the same manner as in Example 1, the solution A2 was coated and filled into each of the mold pores, and then centrifuged (3,000 rpm, 5 20 minutes). Consequently, the solution A2 was filled into the pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. The wrapping film was removed, and residue on the mold surface was removed. Next, the solution B2 was thinly coated over the whole of the mold surface. In addition, the solution 25 C2 was placed over each of the mold pores, and a paper sheet (support) was 31 covered and pasted thereon. The mold was centrifuged by a table-top centrifuge (3,000 rpm, 30 minutes). Consequently, the solution C2 was filled into the pores, and superimposed over a solution A3. Simultaneously, the respective solutions in the mold were dried and solidified. The paper 5 sheet was slowly peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the paper sheet. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing the diclofenac sodium salt and a 10 rear end portion formed from only the base. The acral portions were colored white due to the presence of the diclofenac sodium salt. The length L of the acral portions was approximately 350 rim. Example 3 [00861 An insulin solution having a concentration of 9.6 mg/mL was 15 prepared by dissolving insulin sodium salt (self-prepared product; target substance) in purified water. A 0.1 mL insulin solution was added to 15.9 mg of porous anhydrous silicic acid (trade name: Sylysia 350; Fuji Sylysia Chemical Ltd.; porous substance) (average particle size: 3.9 sm), and the resultant mixture was thoroughly mixed and then dried. Consequently, an 20 insulin-adsorbed powder was obtained in which insulin was held on the porous anhydrous silicic acid. A paste-like base solution was prepared by adding 800 iL of purified water to 300 mg of chondroitin sulfate C sodium salt (Nacalai Tesque, Inc.; base), and thoroughly dissolving and mixing the resultant mixture. A dense solution (solution A3) was then prepared by 25 adding the insulin-adsorbed powder to this base solution, and thoroughly 32 mixing the resultant mixture. Furthermore, an adhesive solution (solution B3) was prepared by adding 35 mL of purified water to 1.5 mg of chondroitin sulfate C sodium salt and 50 mg of Hiviswako 103, and thoroughly dissolving and mixing the resultant mixture. 5 [0087] In the same manner as in Example 1, the solution A3 was coated and filled into each of the mold pores, and then centrifuged (3,000 rpm, 3 minutes). Consequently, the solution A3 was filled into the pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. The wrapping film was removed, 10 and residue on the mold surface was removed. The solution B3 was placed over each of the mold pores, and coated over the whole of the mold surface. Then, the mold was centrifuged by a table-top centrifuge (3,000 rpm, 30 minutes). Consequently, the solution B3 was filled into the pores, and superimposed over the solution A3. Simultaneously, the respective thick 15 liquids in the mold were dried and solidified. A sheet of filter paper (support) moistened with purified water was pasted on the mold surface, then slowly peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the filter paper. Consequently, a patch/microneedle array (preparation for body surface application-holding 20 sheet) holding 100 microneedles (preparations for body surface application) was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing the insulin sodium salt held on the porous anhydrous silicic acid and a rear end portion formed of only the base, from which the insulin sodium salt was 25 to be sustainedly released.
33 Example 4 [0088] A viscous base solution was prepared by adding 20 mL of purified water to 2.0 g of hyaluronic acid (Foodchemifa Co., Ltd., trade name: FCH SU), and then uniformly stirring the resultant mixture with a homogenizer. 5 A dense solution (solution A4) was prepared by dissolving 20 mg of ascorbic acid (Nacalai Tesque, Inc.; target substance) in 50 gL of purified water, then adding 2.1 g of the base solution, and thoroughly mixing the resultant mixture. Furthermore, an adhesive (solution B4) was prepared by adding 1.0 g of the base solution to 1 mg of Hiviswako 103, and thoroughly mixing 10 the resultant mixture. [00891 The solution A4 was degassed. In the same manner as in Example 1, the solution A4 was coated and filled into each of the mold pores, and then centrifuged (3,000 rpm, 5 minutes). Consequently, the solution A4 was filled into the pores more towards the deeper end (tip side) of the pores, so 15 that a space was formed at the near side (rear end side) of the pores. The wrapping film was taken off, and residue on the mold surface was removed. Then, the solution B4 was placed over each of the mold pores, and coated over the whole of the mold surface. The mold was centrifuged by a table-top centrifuge (3,000 rpm, 30 minutes). Consequently, the solution B4 was 20 filled into the pores, and superimposed over the solution A4. Simultaneously, the respective solutions in the mold were dried and solidified. A paper sheet (support) coated with the solution B4 was pasted on the mold surface, then slowly peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the paper sheet. 25 Consequently, a patch/microneedle array holding 100 microneedles was 34 obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing ascorbic acid and a rear end portion formed from only the base. Example 5 5 [0090] A viscous, dense solution (solution A5) was prepared by adding 120 piL of purified water to 7.5 mg of insulin sodium salt (self-prepared product; target substance), 0.2 mg of evans blue, and 52.5 mg of chondroitin sulfate C sodium salt (Wako Pure Chemical Industries, Ltd.; base), and thoroughly dissolving and mixing the resultant mixture. Furthermore, a dense solution 10 (solution B5) was prepared by adding 30 iL of purified water to 30 mg of chondroitin sulfate C sodium salt and 0.5 mg of Hiviswako 103, and thoroughly dissolving and mixing the resultant mixture. In addition, an adhesive (solution C5) was prepared by adding 36 mL of purified water to 1.6 g of Hiviswako 103, and dissolving the resultant mixture. 15 [00911 The solution A5 was put on the tip of a 27G syringe needle, and dispensed into each of the pores of the mold of Example 1 in an atmosphere humidified with water vapor. In the same manner as in Example 1, the surface was covered by a wrapping film, and then the mold was centrifuged (3,000 rpm, 2 minutes). Consequently, the solution A5 was filled into the 20 pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Furthermore, the solution B5 was coated and filled into each of the mold pores (spaces), and centrifuged (3,000 rpm, 5 minutes). Consequently, the solution B5 was filled into the pores, and superimposed over the solution A5. The solution 25 C5 was coated on the surface of a paper sheet (support), then pasted on the 35 surface of the mold. The mold was centrifuged in that state (3,000 rpm, 30 minutes), so that the respective solutions in the mold were dried and solidified. A cloth adhesive bandage (Nichiban (registered trademark); Nichiban Co., Ltd.) was further pasted over the paper sheet, then slowly 5 peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the paper sheet. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing the insulin sodium salt and a rear end portion 10 containing the adhesive substance. The acral portions were colored blue due to the presence of the evans blue. The length L of the acral portions was approximately 200 to 300 pm. Fig. 10 shows a photograph of the microneedle array produced in the present example. In the acral portion of each microneedle (colored black in the photograph) insulin and evans blues 15 are present. [00921 Evaluation of the microneedles in the present example was carried out simultaneously with the following Example 6. Example 6 [00931 A viscous, dense solution (solution A6) was prepared by adding 120 20 gL of purified water to 3.75 mg of insulin sodium salt (self-prepared product; target substance), 0.2 mg of evans blue, and 56.25 mg of chondroitin sulfate C sodium salt (Wako Pure Chemical Industries, Ltd.; base), and thoroughly dissolving and mixing the resultant mixture. A patch/microneedle array holding 100 microneedles was obtained in the same manner as in Example 5, 25 except that the solution A6 was used instead of the solution A5. The length 36 of the acral portions (blue) of the microneedles was approximately 200 to 300 pm. The respective microneedles produced in Examples 5 and 6 were subjected to the following evaluations. [0094] [Measurement of Insulin Content] 5 One hundred microneedles were collected from each patch produced in Examples 5 and 6, and placed in a 1.5 mL capacity sample cup for centrifugal separation. The microneedles were dissolved with 1.0 mL phosphate buffer. One hundred stL of the resultant mixture was subjected to HPLC to measure the insulin content. 10 Then the content per patch (mean value) for each example was calculated. The results were that the patch from Example 5 was 0.70 IU and the patch from Example 6 was 0.37 IU. [0095] [Test Using Rat] Male Wistar rats having the body weight of approximately 350 g was 15 secured to an operating table under the anesthesia with pentobarbital, and the hair from the abdomen was removed. At this stage, first, approximately 0.2 mL of blood was collected from the jugular vein. Next, one patch from Example 5 or 6 was pressed against the abdominal skin of the rat from which hair had been removed to administer insulin to the skin. Blood was 20 collected from the jugular vein for 5 hours after administration, and systemic blood was collected. A serum sample was obtained from each of the obtained blood specimens, and the serum glucose level (blood sugar level) was measured using a glucose assay kit (Glucose C-Il Test Wako; Wako Pure Chemical Industries, Ltd.). The respective blood glucose levels 25 are expressed as the relative value with respect to the pre-dose blood 37 glucose level of 100%. All of the data was calculated as the mean SD of 3 or 4 rats per group. The results are shown in Fig. 11. In Fig. 11, the data indicated with black square are the results for the preparation of Example 5, and the data indicated with white square are the test results for the 5 preparation of Example 6. As is clear from Fig. 11, all of the preparations showed the minimum blood glucose level at 1 hour after administration, and thus the effect of insulin was observed. [00961 Using different group of rats, the insulin solution was administered by subcutaneous injection at 1.0 IU/kg to study the temporal transitions of 10 the hypoglycemic effect. By comparing with the hypoglycemic effect, the pharmacological availability of insulin from each patch/microneedle array was calculated. As a result, the preparation of Example 5 showed 35.7 ± 7.0%, and the preparation of Example 6 showed 36.3 ± 2.6%. It was thus shown that insulin can be administered from the skin with high absorption 15 efficiency by the patch of either Example 5 or 6. Example 7 [0097] A viscous, dense solution (solution A7) was prepared by kneading 46 gL of an erythropoietin injection liquid (trade name: Espo Subcutaneous Injection; 24,000 units/0.5 mL; Kirin Brewery Company Limited; target 20 substance), with 0.5 mg of evans blue, and 45 mg of chondroitin sulfate C sodium salt (base). Furthermore, dense solution (solution B7) was prepared by adding 620 pL of purified water to 600 mg of chondroitin sulfate C sodium salt and 5 mg of Hiviswako 103, and thoroughly dissolving and mixing the resultant mixture. In addition, adhesive solution (solution C7) 25 was prepared by adding 36 mL of purified water to 1.6 g of Hiviswako 103, 38 and thoroughly dissolving and mixing the resultant mixture. [00981 In the same manner as in Example 1, the solution A7 was coated and filled into each of the mold pores, and then centrifuged (4,000 rpm, 5 minutes). Consequently, the solution A7 was filled into the pores more 5 towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Furthermore, the solution B7 was coated and filled into each of the mold pores (spaces), and centrifuged (3,000 rpm, 15 minutes). Consequently, the solution B7 was filled into the pores, and superimposed over the solution A7. Simultaneously, the respective 10 dense solutions in the mold were dried and solidified. The solution C7 was coated on the surface of a paper sheet (support), then pasted on the surface of the mold, and centrifuged in that state (3,000 rpm, 30 minutes) to dry. The paper sheet was slowly peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the paper sheet. 15 Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing erythropoietin (EPO) and a rear end portion containing the adhesive substance. 20 [00991 Evaluation of the microneedles in the present example was carried out simultaneously with the following Example 8. Example 8 [0100] Erythropoietin injection solution was concentrated by a factor of two under a nitrogen gas flow. A viscous, dense solution (solution A8) was 25 prepared by kneading 46 pL of this dense solution, with 0.5 mg of evans 39 blue, and 45 mg of chondroitin sulfate C sodium salt (base). A patch/microneedle array holding 100 microneedles was obtained in the same manner as in Example 7, except that the solution A8 was used instead of the solution A7. Any of the 100 microneedles held on the sheet had two sections 5 as illustrated in Figs. 1 and 2, namely, an acral portion contained EPO and a rear end portion contained the adhesive substance. The respective microneedles produced in Examples 7 and 8 were subjected to the following evaluations. [0101] [Measurement of EPO Content] 10 One hundred microneedles were collected by the same procedure as in Example 6, and the EPO content (mean value) per patch produced in Examples 7 and 8 was calculated. The EPO content was measured using an EPO Elisa Kit (Roche Diagnostics KK). As the results, the patch from Example 7 had an EPO content of 12.5 ± 1.5 IU and the patch from Example 15 8 had an EPO content of 31.3 ± 5.9 IU. [01021 [Rat Experiments] The experiment was carried out basically by the same procedures as in Example 6. Three or four rats were used per group. Blood was collected from the jugular vein for 24 hours after EPO administration, and the 20 systemic blood was collected. Using the EPO Elisa Kit, the serum EPO concentrations were measured. The results are shown in Fig. 12. In Fig. 12, the data indicated by black square are the results for the preparation of Example 7 (low dose group), and the data indicated by white square are the results for the preparation of Example 8 (high dose group). As is clear from 25 Fig. 12, all of the preparations showed an increase in the serum EPO level 40 in proportion with the EPO content in the microneedles. Thus, a good dose dependency was obtained. [0103] Using different group of rats, the EPO injection solution was administered by subcutaneous injection at the dose of 1.0 IU/kg. The mean 5 value of the area under the serum EPO level-time curve (AUC) after administration was determined, and the bioavailability was calculated. As the result, the preparation of Example 7 (low dose group) had 30% as the mean value, and the preparation of Example 8 (high dose group) had the mean value of 29%. It was thus shown that EPO can be administered from 10 the skin with high absorption efficiency by the microneedles of either Example 7 or 8. Example 9 [0104] Egg albumin (OVA) was employed as a model antigen. A solution was made by adding 9.0 mL of purified water to 4.0 mg of egg albumin (egg 15 albumin (crude); Nacalai Tesque, Inc.; target substance) and 5.0 mg of evans blue to dissolve. A viscous, dense solution (solution A9) was prepared by adding 8.5 g of chondroitin sulfate C sodium salt to the above solution. Further, dense solution (solution B9) was prepared by adding 1.0 mL of purified water to 1.0 mg of chondroitin sulfate C sodium salt and 0.5 mg of 20 Hiviswako 103, and thoroughly dissolving and mixing the resultant mixture. [0105] The solution A9 was put on the tip of a 27G syringe needle, and dispensed into each of the pores of the mold of Example 1 in an atmosphere humidified with water vapor. The mold was placed in an acrylic resin case, and then centrifuged (3,000 rpm, 3 minutes) in the same manner as in 25 Example 1. Consequently, the solution A9 was filled into the pores more 41 towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. The mold was taken out of the case, and residue on the mold surface was removed. Furthermore, the solution B9 was coated on each of the mold pores (spaces). A paper sheet 5 (support) was placed over the mold, and both ends of the sheet were fixed by a cloth adhesive bandage. Then, the mold was centrifuged (3,000 rpm, 30 minutes). Consequently, the solution B9 was filled into the pores, and superimposed over the solution A9. Simultaneously, the respective dense solution in the mold were dried and solidified. The paper sheet was slowly 10 peeled off, so that the needle-shaped solid stuff was removed from the mold while still held on the paper sheet. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing OVA and a rear end portion containing the 15 adhesive substance. The acral portions were colored blue due to the presence of the evans blue. The length L of the acral portions was approximately 300 to 350 im. [0106] Five BALB/c mice having body weight of approximately 30 g were used as one group. The mice were secured to an operating table under 20 anesthesia with pentobarbital, and the hair from their backs was removed. Next, one patch from the present example was pressed against the backs of the mice whose hair had been removed to administer OVA from the skin. Two weeks after administration, OVA was again administered using one patch. Two weeks after the second administration, all of the blood was 25 collected. As a positive control group, OVA was administered as an aqueous 42 solution by subcutaneous injection to a second group of different mice at the dose of 1.0 microgram (Comparative Example 1) or 0.1 microgram (Comparative Example 2) at the zero week and second week, and similarly all of the blood was collected after 2 weeks had elapsed from the second 5 administration. Using the obtained serum specimens, the OVA antibody titer was measured. The results were that when the microneedles obtained in the present example were administered, an antibody titer between that of Comparative Example 2 (subcutaneous injection of 0.1 micrograms) and Comparative Example 1 (subcutaneous injection of 1.0 microgram) was 10 shown. Example 10 [01071 A standard buffer (Nacalai Tesque, Inc.) having a pH of 4.01 was diluted by a factor of 10 with purified water (dilute buffer). Then, 5.0 mg of pilocarpine hydrochloride (Nacalai Tesque, Inc.) was dissolved in 10 mL of 15 the above dilute buffer and 4.0 mL of ethyl alcohol. Furthermore, 500 mg of hydroxypropyl methylcellulose phthalate (HPMCP; Variety HP-55S; Shin Etsu Chemical Co. Ltd.; base) was added, and the resultant mixture was stirred at about 40*C to dissolve. After dissolving, the mixture was further stirred under warm air to concentrate to the viscosity at which the mixture 20 could be easily coated on the mold (solution A10). Furthermore, dense solution (solution B10) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and thoroughly dissolving and mixing the resultant mixture. [0108] In the same manner as in Example 1, the solution A10 was coated 25 and filled into each of the mold pores. In the same manner as in Example 9, 43 the mold was placed in an acrylic resin case, and then centrifuged (3,000 rpm, 30 minutes). Consequently, the solution A10 was filled into the pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Furthermore, in the 5 same manner as in Example 9, the solution B 10 was coated and filled into each of the mold pores (spaces), and centrifuged (3,500 rpm, 5 minutes). Consequently, the solution B10 was filled into the pores, and superimposed over the solution A10. The mold was moved to a desiccator, so that the respective dense solutions in the mold were dried and solidified. The 10 needle-shaped solid stuff was removed from the mold to obtain 100 microneedles. Any of the 100 microneedles had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing pilocarpine and a rear end portion containing chondroitin sulfate C sodium salt. [0109] Under ether anesthesia, 20 microneedles from the present 15 examples were inserted into the eyeball cornea of rabbits, and the state of the pupil was observed. As a result, pupil constriction effect appeared at 30 minutes after administration and the maximum miotic rate was 63%. Example 11 [0110] A dense solution (solution All) was prepared by adding 10 pL of 20 sumatriptan (trade name: Imigrane Nasal Drops; target substance; equivalent to 2.0 mg of sumatriptan) and 140 gL of purified water to 0.5 mg of methylene blue (Nacalai Tesque, Inc.) and 5.0 mg of hyaluronic acid (trade name: FCH-60; Foodchemifa Co., Ltd.; base), and thoroughly dissolving and mixing the resultant mixture. Further, dense solution 25 (solution B11) was prepared by adding 1.0 mL of degassed purified water to 44 1.0 g of high molecular weight dextran (Nacalai Tesque, Inc.). [0111] In the same manner as in Example 9, the solution All was dispensed into each of the mold pores, and then centrifuged (3,500 rpm, 15 minutes). Consequently, the solution All was filled into the pores more 5 towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. The mold was taken out of the case, and residue on the mold surface was removed. The mold was further centrifuged (3,500 rpm, 15 minutes). Subsequently, in the same manner as in Example 9, coating of the solution B11, pasting and centrifuging of the 10 paper sheet, and drying were carried out. After the drying, the paper sheet was slowly peeled off and the needle-shaped solid stuff on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an 15 acral portion containing sumatriptan and a rear end portion containing the high molecular weight dextran. The acral portions were colored blue due to the presence of the methylene blue. The length L of the acral portions was approximately 300 to 350 pm. [0112] Male Wistar rats (3 or 4 rats) having the body weight of 20 approximately 330 g were secured to an operating table under anesthesia with pentobarbital, and then the hair from their abdomen was removed. Approximately 0.2 mL of blood was collected from the jugular vein, and then one patch produced in the present example was pressed against the abdominal skin of the rats whose hair had been removed to administer 25 sumatriptan from the skin. Blood was collected from the jugular vein for 3 45 hours after administration, and systemic blood was collected. Plasma samples were obtained by centrifugation, and the plasma sumatriptan concentrations were measured by an LC/MS/MS method. The results are shown in Table 1. The values in the table are the mean values of 3 to 4 5 experiments. Specifically, a good plasma sumatriptan levels were obtained by transdermal administration.
00 0 0.C N ~ '-4 3 010 0c 0 C.) C. cqo 0 0 47 Example 12 [0113] A viscous, dense solution (solution A12) was prepared by adding 90 pL of degassed purified water to 5.0 mg of recombinant human growth hormone (Wako Pure Chemical Industries, Ltd.; target substance), 35 mg of 5 chondroitin sulfate C sodium salt, and 0.5 mg of lissamine green B (MP Biomedicals LLC), and thoroughly dissolving and mixing the resultant mixture. Further, dense solution (solution B 12) was prepared by adding 1 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and thoroughly dissolving and mixing the resultant mixture. 10 [01141 In the same manner as in Example 1, the solution A12 was coated and filled into each of the mold pores. In the same manner as in Example 9, the mold was placed in an acrylic resin case, and then centrifuged (3,500 rpm, 10 minutes). The mold was taken out from the case, and centrifuged further (3,500 rpm, 5 minutes). Consequently, the solution A12 was filled 15 into the pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Next, the solution B12 was coated and filled into each of the mold pores (spaces), and also coated on the mold surface. A paper sheet was pasted on the mold surface, and both ends were fixed by a tape. Then, the mold was centrifuged 20 (3,500 rpm, 30 minutes). Consequently, the solution B12 was filled into the pores, and superimposed over the solution A12. Simultaneously, the respective dense solutions in the mold were dried and solidified. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a 25 patch/microneedle array holding 100 microneedles was obtained. Any of the 48 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing human growth hormone and a rear end portion. The length L of the tip portions was approximately 250 pm. 5 [0115] In the same manner as in Example 1, one patch of the present example was pressed against the skin of 2 rats to administer human growth hormone. Blood was collected from the jugular vein for 4 hours after administration, and systemic blood was collected. Plasma samples were obtained by centrifugation, and the plasma human growth hormone level in 10 each sample was measured by an hGH-Elisa Kit (Biosource). The results are shown in Table 2. The values in the table are the mean value of 2 experiments. The area under the plasma drug concentration-time curve, AUC, was obtained and compared with the AUC value obtained by intravenous study of hGH to calculate bioavailability. A value of 15 approximately 90% was obtained. [Table 21 Time (min) 0 15 30 45 60 90 120 180 240 Growth hormone ND1 32.4 31.6 28.2 23.8 16.6 12.8 5.0 2.3 concentration (ng/mL) ND: Not detected Example 13 [0116] A viscous, dense solution (solution A13) was prepared by adding 50 20 gL of degassed purified water to 5.0 mg of tacrolimus (FK506; Sigma; target substance) which had been subjected to fine pulverization using a mortar made from agate, 0.5 mg of evans blue, and 25 mg of chondroitin sulfate C sodium salt, and thoroughly mixing the resultant mixture. Further, dense 49 solution (solution B13) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and dissolving and kneading the resultant mixture. In addition, another dense solution (solution C13) was prepared by adding 1.5 mL of degassed purified water to 5 1.0 g of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. [0117] The solution C13 was put on the tip of a 27G syringe needle, coated on each of the mold pores, and dried while centrifuging (3,000 rpm, 15 minutes). Consequently, the solution C13 was filled into the pores more 10 towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Then, in the same manner as in Example 1, the solution A13 was coated and filled into each of the mold pores. In the same manner as in Example 9, the mold was placed in an acrylic resin case, and then centrifuged (3,500 rpm, 15 minutes). The mold 15 was taken out from the case, and centrifuged further (3,500 rpm, 5 minutes). Consequently, the solution A13 was filled into the pores, and superimposed over the solution C13. However, a space was left on the near side (rear end side) of the pores. Next, the solution B13 was coated and filled into each of the mold pores (spaces), and also coated on the mold surface. A paper sheet 20 was pasted on the mold surface, and both ends were fixed by a tape. Then, the mold was centrifuged (3,500 rpm, 20 to 30 minutes). Consequently, the solution B 13 was filled into the pores, and superimposed over the solution A13. Simultaneously, the respective dense solutions in the mold were dried and solidified. The paper sheet was slowly peeled off and the needle-shaped 25 solid stuff held on the paper sheet was removed from the mold.
50 Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had three sections as illustrated in Figs. 5 and 6, namely, a tip portion formed from the base, a middle portion containing tacrolimus, and a rear end portion. The middle 5 portions were colored blue due to the presence of the evans blue. [0118] In the same manner as in Example 1, one patch of the present example was pressed against the skin of 2 rats to administer tacrolimus. Blood was collected from the jugular vein for 24 hours after administration, and systemic blood was collected. Plasma sample was prepared from each of 10 the obtained blood sample. Tacrolimus was extracted from plasma sample by solid extraction method and was measured using LC/MS/MS. The results are shown in Table 3. The values in the table are the mean value of 2 examples. The results show that while tacrolimus was detected in the plasma, its concentrations were very low. Calculating the bioavailability by 15 comparing with the area under the plasma tacrolimus level-time curve, AUC, obtained after intravenous injection of tacrolimus gave a value of approximately 0.3%. It was thought that tacrolimus was delivered to a site near the skin after administration to the skin. [Table 31 Time (hr) 0 1 2 3 4 5 6 9 12 24 Tacrolimus ND 0.4 0.6 0.6 0.5 0.5 00.5 .5 0.5 0.5 concentration (ng/mL) 20 ND: Not detected Example 14 [01191 1.0 mg of desmopressin (DDAVP; Wako Pure Chemical Industries, Ltd.; target substance) was dissolved in 50 pL of a pH 6.5 phosphate buffer.
51 Then, a viscous, dense solution (solution A14) was prepared by further adding 0.5 mg of evans blue and 25 mg of chondroitin sulfate C sodium salt, and mixing the resultant mixture. Further, viscous solution (solution B14) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of 5 chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. [01201 In the same manner as in Example 1, the solution A14 was coated and filled into each of the mold pores. Subsequently, by the same procedures as in Example 13, centrifuging (3,500 rpm, 15 minutes), 10 centrifuging (3,500 rpm, 20 minutes), coating of the solution B14, pasting of the paper sheet, and centrifuging (3,500 rpm, 20 to 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 15 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, acral portion containing desmopressin and a rear end portion. The acral portions were colored blue due to the presence of evans blue. [01211 In the same manner as in Example 1, one patch of the present example was pressed against the skin of 3 to 4 rats to administer 20 approximately 10 sg/kg of desmopressin. Blood was collected from the jugular vein for 6 hours after administration, and systemic blood was collected. Plasma sample was prepared from each of the obtained blood sample. Desmopressin in each plasma sample was extracted by solid phase extraction method, and its concentration was measured using LC/MS/MS. 25 As a control, desmopressin was intravenously administered to different 52 group of rats, 15 gg/kg. The results are shown in Fig. 13. In Fig. 13, the data indicated by a black circle are the experimental results for the case when the preparation of the present example was transdermally administered, and the data indicated by a black square are the experimental 5 results for the case when desmopressin was intravenously administered. The values in the graph show the mean SD of 3 to 4 experiments. Specifically, when the preparation of the present example was administered, the percutaneous absorption efficiency was approximately 100%. Example 15 10 [01221 A viscous, dense solution (solution A15) was prepared by adding 100 sL of degassed purified water to 10.0 mg of heparin sodium salt (Nacalai Tesque, Inc.; target substance), 0.5 mg of evans blue, and 35 mg of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. Further, a viscous solution (solution B15) was prepared by adding 15 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. [01231 By the same procedures as in Example 14, coating of the solution A15 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B15, pasting of the paper 20 sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 25 and 2, namely, a tip portion containing heparin and a rear end portion. The 53 acral portions were colored blue due to the presence of the evans blue. The length L of the acral portions was approximately 300 Am. Example 16 [01241 Rifampicin (Wako Pure Chemical Industries, Ltd.; target 5 substance) was pulverized using an agate mortar. A viscous, dense solution was prepared by adding 65 pL of degassed purified water to 0.5 mg of evans blue and 25 mg of chondroitin sulfate C sodium salt, and mixing the resultant mixture. A dense suspension (solution A16) was prepared by adding 5.0 mg of the pulverized rifampicin product to the above dense 10 solution. Further, a viscous solution (solution B 16) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. In addition, another viscous solution (solution C16) was prepared by adding 1.5 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and dissolving 15 and mixing the resultant mixture. [01251 By the same procedures as in Example 13, coating of the solution C16 into each pore, centrifuging and drying, coating of the solution A16 into each pore, centrifuging (3,500 rpm, 15 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B16, pasting of the paper sheet, and 20 centrifuging (3,500 rpm, 20 to 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had three sections as illustrated in Figs. 25 5 and 6, namely, an acral portion composed from the base, a middle portion 54 containing rifampicin, and a rear end portion. Fig. 14 shows a photograph of the obtained microneedle array. [01261 In the same manner as in Example 1, one patch of the present example was pressed against the skin of 2 rats to administer rifampicin. 5 Blood was collected from the jugular vein for 12 hours after administration, and systemic blood was collected. Plasma sample was prepared from each of the obtained blood sample. Rifampicin was extracted from the plasma sample by solid phase extraction method, and the concentration was measured using LC/MS/MS. The results are shown in Table 4. The values 10 in the table are the mean value of 2 experiments. The results show that rifampicin was detected in the plasma. [Table 41 Time (hr) 0 1 2 3 4 5 6 8 12 Rifampicin ND1 9.1 10.2 4.8 2.8 2.7 1.5 1.4 1.1 concentration (ng/mL) ND: Not detected Example 17 15 [0127] A viscous, dense solution (solution A17) was prepared by adding 40 gL of degassed purified water to 2.5 mg of leuprorelin acetate (Techno Science Japan Co., Ltd.; target substance), and 10.0 mg of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. Further, a viscous solution (solution B17) was prepared by adding 750 RL of 20 degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and dissolving and mixing the resultant mixture. [0128] By the same procedures as in Example 14, coating of the solution A17 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging 55 (3,500 rpm, 5 minutes), coating of the solution B 17, pasting of the paper sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a 5 patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing leuprorelin acetate and a rear end portion. [0129] In the same manner as in Example 1, one patch of the present 10 example was pressed against the skin of 2 rats to administer leuprorelin acetate. Blood was collected from the jugular vein for 4 hours after administration, and the systemic blood was collected. Plasma samples were prepared from the obtained blood samples. Leuprorelin acetate was extracted from the plasma sample by solid phase extraction method and the 15 concentration was measured using LC/MS/MS. The results are shown in Table 5. The values in the table are the mean values of 2 examples. Specifically, good transdermal absorption of leuprorelin was shown. [Table 51 Time (min) 0 15 30 60 120 180 240 Leuprorelin ND 10.3 12.7 5.3 1.4 0.6 0.3 concentration (ng/mL) ND: Not detected 20 Example 18 [01301 A viscous, dense solution (solution A18) was prepared by adding 80 sL of degassed purified water to 5.0 mg of recombinant human growth hormone (Wako Pure Chemical Industries, Ltd.; target substance), 0.5 mg of 56 lissamine green B, and 35 mg of high molecular weight dextran (base), and thoroughly dissolving and mixing the resultant mixture. Further, a viscous solution (solution B18) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of high molecular weight dextran, and thoroughly dissolving 5 and mixing the resultant mixture. [01311 By the same procedures as in Example 14, coating of the solution A18 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B18, pasting of the paper sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper 10 sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing human growth hormone and a 15 rear end portion. The acral portions were colored green due to the presence of the lissamine green B. The length L of the acral portions was approximately 250 gm. Example 19 [01321 A viscous, dense solution (solution A19) was prepared by adding 20 200 gL of degassed purified water to 0.5 mg of human basic fibroblast growth factor (bFGF; trade name: Fiblast Spray; Kaken Pharmaceutical Co., Ltd.; target substance) and 100 mg of pullulan (trade name: Pullulan PI-20; Hayashibara Biochemical Labs., Inc; base), and thoroughly dissolving and mixing the resultant mixture. Further, a viscous solution (solution B 19) 25 was prepared by adding 3.0 mL of degassed purified water to 1.5 g of 57 pullulan, and thoroughly dissolving and mixing the resultant mixture. [01331 By the same procedures as in Example 14, coating of the solution A19 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B19, pasting of the paper 5 sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 10 and 2, namely, a tip portion containing human bFGF and a rear end portion. Example 20 [0134] A solution A19 (bFGF + pullulan) was prepared in the same manner as in Example 19. Lymphatic fluid was collected by cannulation of the thoracic lymph duct of rats who had been ingested with bovine milk 15 previously. A lipid dispersion (solution A20) was prepared by adding 100 sL of this lymphatic fluid to the solution A20, and thoroughly mixing the resultant mixture. Further, a viscous solution (solution B20) was prepared by adding 3.0 mL of degassed purified water to 1.5 g of pullulan, and thoroughly dissolving and mixing the resultant mixture. 20 [01351 By the same procedures as in Example 14, coating of the solution A20 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging (2,000 rpm, 5 minutes), coating of the solution B20, pasting of the paper sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the 25 paper sheet was removed from the mold. Consequently, a 58 patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, a tip portion containing human bFGF (forming a complex with the lipids) and a rear end portion. 5 Example 21 [0136] A viscous, dense solution was prepared by adding 200 pL of degassed purified water to 200 mg of high molecular weight dextran (Nacalai Tesque, Inc.; base). On the other hand, blood was separated by centrifugation, and the supernate, plasma, was collected. Then, the red 10 blood cell (target substance) fraction was carefully collected. 100 .L of the red blood cell fraction was added to a dense solution of high molecular weight dextran, and was mixed (solution A21). Furthermore, a viscous solution (solution B21) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of high molecular weight dextran, and thoroughly dissolving 15 and mixing the resultant mixture. [0137] By the same procedures as in Example 13, coating of the solution A21 into each pore, centrifuging (3,500 rpm, 10 minutes), centrifuging (3,500 rpm, 20 minutes), coating of the solution B21, pasting of the paper sheet, and centrifuging (3,500 rpm, 20 to 30 minutes) were carried out. The 20 paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, a tip portion containing red blood cells and a rear end 25 portion.
59 Example 22 [0138] A viscous, dense solution was prepared by adding 50 gL of distilled water to 0.5 mg of evans blue and 25 mg of chondroitin sulfate C sodium salt (base), and thoroughly dissolving and mixing the resultant mixture. 5 Suspension (solution A22) was prepared by adding 5.0 mg of leuprorelin microcapsules (trade name: Leuplin for Injection 1.88; Takeda Pharmaceutical Company Limited; target substance) to the above thick liquid, and thoroughly mixing the resultant mixture. Further, dense solution (solution B22) was prepared by adding 750 gL of degassed purified 10 water to 1.0 g of chondroitin sulfate C sodium salt, and thoroughly dissolving and mixing the resultant mixture. In addition, another viscous solution (solution C22) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and thoroughly dissolving and mixing the resultant mixture. 15 [01391 By the same procedures as in Example 13, coating of the solution C22 into each pore, centrifuging and drying, coating of the solution A22 into each pore, centrifuging (3,500 rpm, 5 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B22, pasting of the paper sheet, and centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was 20 slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had three sections as illustrated in Figs. 5 and 6, namely, an acral portion made from the base, a middle portion containing leuprorelin 25 microcapsules, and a rear end portion. The middle portions were colored 60 blue due to the presence of evans blue. Example 23 [0140] A viscous, dense solution was prepared by adding 50 sL of distilled water to 0.5 mg of evans blue and 25 mg of high molecular weight dextran 5 (base), and thoroughly dissolving and mixing the resultant mixture. Suspension (solution A23) was prepared by adding 5.0 mg of leuprorelin microcapsules (trade name: Leuplin for Injection 1.88; Takeda Pharmaceutical Company Limited; target substance) to the above thick liquid, and thoroughly mixing the resultant mixture. Furthermore, an 10 adhesive solution (solution B23) was prepared by adding 750 sIL of degassed purified water to 750 mg of high molecular weight dextran, and thoroughly dissolving and mixing the resultant mixture. In addition, a viscous solution (solution C23) was prepared by adding 1.0 mL of degassed purified water to 750 mg of high molecular weight dextran, and thoroughly dissolving and 15 mixing the resultant mixture. [0141] By the same procedures as in Example 13, coating of the solution C23 into each pore, centrifuging and drying, coating of the solution A23 into each pore, centrifuging (3,500 rpm, 5 minutes), centrifuging (3,500 rpm, 5 minutes), coating of the solution B23, pasting of the paper sheet, and 20 centrifuging (3,500 rpm, 30 minutes) were carried out. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had three sections as illustrated in Figs. 5 and 6, namely, an 25 acral portion formed from the base, a middle portion containing leuprorelin 61 microcapsules, and a rear end portion. The middle portions were colored blue due to the presence of the evans blue. Example 24 [01421 A solution was prepared by adding 1.0 mL of purified water to 1.0 g 5 of liposomal amphotericin B preparation (trade name: AmBisome; Dainippon Sumitomo Pharma Co., Ltd.) as a representative of a lipid dispersion preparation, and dissolving the resultant mixture by thoroughly shaking. Then, a viscous, dense solution (solution A24) was prepared by adding 0.7 g of chondroitin sulfate C sodium salt, and thoroughly mixing the 10 resultant mixture. Further, a base solution (solution B24) was prepared by adding 1.0 mL of degassed purified water to 1.0 g of chondroitin sulfate C sodium salt, and thoroughly dissolving and mixing the resultant mixture. [0143] A patch/microneedle array holding 100 microneedles was obtained in the same manner as in Example 5, except that the solution A24 was used 15 instead of the solution A5, and the solution B24 was used instead of the solution B5. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing liposomal amphotericin B and a rear end portion. Example 25 20 [01441 A viscous, dense solution (solution A25) was prepared by adding 40 sL of a 0.1 N sodium hydroxide solution and 30 piL of 0.15% evans blue to 7.5 mg of insulin sodium salt (self-prepared product; target substance), 2.5 mg of heparin sodium salt (Nacalai Tesque, Inc.), and 15 mg of dextran sulfate sodium salt (Wako Pure Chemical Industries, Ltd.; base), and 25 thoroughly dissolving and mixing the resultant mixture. Further, a dense 62 solution (solution B25) was prepared by adding 30 gL of purified water to 30 mg of dextran sulfate sodium salt, and thoroughly dissolving and mixing the resultant mixture. [01451 A patch/microneedle array holding 100 microneedles was obtained 5 in the same manner as in Example 5, except that the solution A25 was used instead of the solution A5, and the solution B25 was used instead of the solution B5. Any of the 100 nicroneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing insulin sodium salt and a rear end portion. Fig. 15 shows a photograph of the 10 obtained microneedle array. [01461 Evaluation of the microneedles in the present example was carried out simultaneously with the following Example 26. Example 26 [0147] A viscous, dense solution (solution A26) was prepared by adding 30 15 pL of purified water to 10.0 mg of insulin sodium salt (self-prepared product; target substance) and 20 mg of chondroitin sulfate C sodium (Wako Pure Chemical Industries, Ltd.; base), and thoroughly dissolving and mixing the resultant mixture. Furthermore, a dense solution (solution B26) was prepared by adding 30 sL of purified water to 30 mg of chondroitin sulfate C 20 sodium, and thoroughly dissolving and mixing the resultant mixture. [01481 A patch/microneedle array holding 100 microneedles was obtained in the same manner as in Example 5, except that the solution A26 was used instead of the solution A5, and the solution B26 was used instead of the solution B5. Any of the 100 microneedles held on the sheet had two sections 25 as illustrated in Figs. 1 and 2, namely, an acral portion containing insulin 63 sodium salt and a rear end portion. [01491 An evaluation based on the rate of hypoglycemic effect in rats was carried out in the same manner as in Example 6 using the patches obtained in Examples 25 and 26. The results showed that the minimum blood 5 glucose level after administration of the patch of Example 26 to the shaved abdominal skin of rats were obtained at about 4 hour after administration. On the other hand, for the patch of Example 25, the minimum blood glucose level was obtained at 1 hour after administration. This is considered that since the association of the insulin molecules occurs when the insulin 10 content in the patch was increased, the dissolution/release rate after administration to the skin was decreased. However, by adding heparin and dextran sulfate sodium salt, the association of insulin molecules was decreased, so that the dissolution/release rate of insulin from the microneedle patch could be increased. 15 Example 27 [0150] A solution A2 and a solution B2 were prepared in the same manner as in Example 2. Further, a dense solution (solution C2) was prepared by adding 1.0 mL of purified water to 300 mg of chondroitin sulfate C sodium salt, and thoroughly dissolving the resultant mixture. 20 [0151] The solution C2 was put on the tip of a 27G syringe needle, coated on each of the mold pores, and dried while centrifuging (3,000 rpm, 15 minutes). Consequently, the solution C2 was filled into the pores more towards the deeper end (tip side) of the pores, so that a space was formed at the near side (rear end side) of the pores. Then, in the same manner as in 25 Example 1, the solution A2 was coated and filled into each of the mold pores, 64 and then centrifuged (3,000 rpm, 5 minutes). Consequently, the solution A2 was filled into the pores, and superimposed over the solution C2. However, a space was left on the near side (rear end side) of the pores. The wrapping film was taken off, and residue on the mold surface was removed. Next, the 5 solution B2 was thinly coated over the whole of the mold surface. In addition, the solution B2 was placed over each of the mold pores, and a paper sheet (support) was covered and pasted thereon. The mold was centrifuged by a table-top centrifuge (3,000 rpm, 30 minutes). Consequently, the solution B2 was filled into the pores, and superimposed over the solution 10 A2. Simultaneously, the respective solutions in the mold were dried and solidified. The paper sheet was slowly peeled off and the needle-shaped solid stuff held on the paper sheet was removed from the mold. Consequently, a patch/microneedle array holding 100 microneedles was obtained. Any of the 100 microneedles held on the sheet had three sections 15 as illustrated in Figs. 5 and 6, namely, an acral portion formed from the base, a middle portion containing diclofenac sodium, and a rear end portion formed from only the base. The middle portions were colored white due to the presence of the diclofenac sodium. The total length Li of the acral portion and the middle portion was approximately 350 Am. 20 Example 28 [0152] In the present example, a comparative experiment was carried out between microneedles holding insulin in an acral portion only and conventional microneedles holding insulin in the whole preparation. [0153] A patch/microneedle array holding 100 microneedles whose acral 25 portions had a length of approximately 300 pm was obtained in the same 65 manner as in Example 1. As a reference sample, using the same mold, a conventional patch/microneedle array was produced which held insulin in the whole preparation. The dimensions of each microneedle were accurately measured. Furthermore, the insulin content per patch was measured. The 5 results are shown in Table 6. Refer to Fig. 2 regarding the total length H of the preparation, the diameter D of the pressing end, and the length L of the acral portion. Each value is the mean value of 100 microneedles. Specifically, the example and the reference sample had basically the same outer dimensions. Further, the example (1.7 ± 0.2 jg/patch) had an insulin 10 content of about 29% that of the reference sample (5.9 ± 0.4 jg/patch). [Table 61 H (sm) D (pm) L (sm) Insulin content (gg/patch) Example 492.6 ± 2.4 290.0 ± 3.6 316.0 ± 7.3 1.7 ± 0.2 Comparative 483.4 ± 4.7 292.2 ± 2.9 - 5.9 ± 0.4 example [0154] An experiment was carried out by the same procedures as in Example 6 using rats, and the hypoglycemic effects for 5 hours after administration were measured. The results showed that, for the 15 microneedles of the example, the total blood glucose decrease area (1 to 5 hours) was 149.7 ± 8.0 % hr, and for the microneedles of the reference sample, the value was 159.8 ± 30.6 % hr. By a statistical analysis using a significance test, no significant difference was found out between the two preparations. Based on the above results, it was shown that the 20 microneedles of the example having lower insulin content (approximately 29% of that contained in the reference sample) showed the same pharmacological effect as the microneedles of the reference sample 66 [01551 Furthermore, the pharmacological availability was calculated to be 30.7 ± 1.9% for the microneedles of the example and 9.2 ± 1.6% for the microneedles of the reference sample. Accordingly, the microneedles of the example were superior in this point too. 5 Example 29 [01561 In the present example, a comparative study was carried out between microneedles holding erythropoietin in the acral portion only and conventional microneedles holding erythropoietin in the whole preparation. [0157] Erythropoietin injection solution was concentrated by a factor of 10 two under the flow of nitrogen gas. A viscous, dense solution (solution A29) was prepared by kneading 46 tL of thus obtained dense solution, 0.5 mg of evans blue, 22.5 mg of chondroitin sulfate C sodium salt (base), and 22.5 mg of high molecular weight dextran. A patch/microneedle array holding 100 microneedles was obtained in the same manner as in Example 7, except that 15 the solution A29 was used instead of the solution A7. Any of the 100 microneedles held on the sheet had two sections as illustrated in Figs. 1 and 2, namely, an acral portion containing EPO and a rear end portion containing the adhesive substance. As a reference experiment, using the same mold, a conventional patch/microneedle array holding 100 20 microneedles which held erythropoietin in the whole preparation was produced.. [01581 An experiment was carried out using 3 rats per group by the same procedures as in Example 8. Blood was collected from the jugular vein for 24 hours after administration to measure the changes in EPO levels in the 25 serum. The results are shown in Fig. 16. In Fig. 16, the black diamond 67 shape indicates the data for the microneedle array (patch) of the example, and the white diamond shape indicates the data for the microneedle array (patch) of the reference experiment. The value of the area under the blood EPO level-time curve AUC was 667.1 + 125.1 (SE) mIU -hr/mL for the 5 example, and 648.0 ± 91.7 (SE) mIU hr/mL for the reference experiment. No significant difference was detected. The results of the content experiment showed that the example preparation containing EPO in the tip portions contained 20.6 ± 5.1 IU. The EPO content for the reference experiment preparation was 102 ± 20.9 IU. From the above result, it was 10 shown that the microneedles of the example containing EPO in the acral portions with a lower erythropoietin content exhibited the same pharmacokinetics as that of the microneedles of the reference experiment which contained EPO throughout. Example 30 15 [0159] Based on the method of Example 1, a total of 4 kinds of microneedles were prepared whose total lengths H were 200, 300, 400, and 500 pm, respectively. These microneedles were inserted into the skin of the arm by pressing with a finger. The results were that there was no blood leakage or pain for any of the microneedles.
Claims (25)
1. A needle-shaped preparation for body surface application, comprising a base formed from a biosoluble substance and a target substance held in the base, the preparation for body surface application 5 being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the preparation for body surface application is formed of two or more sections divided in the insertion direction; the target substance is held in at least one section other than the rearmost 10 end section; and the section in which the target substance is held is obtained by solidifying the base in which the target substance is dissolved.
2. A needle-shaped preparation for body surface application, comprising a base formed from a biosoluble substance and a target 15 substance held in the base, the preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the preparation for body surface application is formed of two or more sections divided in the insertion direction; 20 the target substance is held in at least one section other than the rearmost end section; and the section in which the target substance is held is obtained by solidifying (a) the base in which cells are dispersed, (b) the base in which the target substance is dispersed as a lipid 25 dispersion, or 69 (c) the base in which the target substance formed from fine particles having an average particle size of 10 micrometers or less is dispersed.
3. The preparation for body surface application according to claim 1 or 2, wherein the target substance is held in the frontmost end section. 5
4. The preparation for body surface application according to any of claims 1 to 3, wherein the total length in the insertion direction is in a range of 200 to 600 micrometers.
5. The preparation for body surface application according to claim 4, wherein the total length in the insertion direction is in a range of 400 to 600 10 micrometers.
6. The preparation for body surface application according to claim 5, wherein a sum of the lengths in the insertion direction of the sections excluding the rearmost end section is 350 micrometers or less.
7. A needle-shaped preparation for body surface application, 15 comprising a base formed from a biosoluble substance and a target substance held in the base, the preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the target substance is not uniformly distributed in the base along the 20 insertion direction with more of the target substance present towards a tip side than a rear end side; and the portion in which the target substance is present is obtained by solidifying the base in which the target substance is dissolved.
8. A needle-shaped preparation for body surface application, 25 comprising a base formed from a biosoluble substance and a target 70 substance held in the base, the preparation for body surface application being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the target substance is not uniformly distributed in the base along the 5 insertion direction with more of the target substance present towards a tip side than a rear end side; and the portion in which the target substance is present is obtained by solidifying (a) the base in which cells are dispersed, 10 (b) the base in which the target substance is dispersed as a lipid dispersion, or (c) the base in which the target substance formed from fine particles having an average particle size of 10 micrometers or less is dispersed.
9. The preparation for body surface application according to claim 7 15 or 8, wherein the total length in the insertion direction is in a range of 200 to 600 micrometers.
10. The preparation for body surface application according to claim 9, wherein the total length in the insertion direction is in a range of 400 to 600 micrometers. 20
11. The preparation for body surface application according to claim 10, wherein the target substance is held in a portion within 350 micrometers from the tip towards the rear end.
12. A needle-shaped preparation for body surface application, comprising a base formed from a biosoluble substance and a target 25 substance held in the base, the preparation for body surface application 71 being used by being inserted into a body surface, and the target substance being absorbed into the body by dissolution of the base, wherein the preparation for body surface application is formed of three or more sections divided in the insertion direction; 5 the target substance is held in at least one section which is not either the frontmost end section or the rearmost end section; and the section in which the target substance is held is obtained by solidifying the base in which the target substance is dispersed.
13. The preparation for body surface application according to claim 10 12, wherein the target substance is held in a section adjacent to the frontmost end section.
14. The preparation for body surface application according to claim 12 or 13, wherein the total length in the insertion direction is in a range of 200 to 600 micrometers.
15 15. The preparation for body surface application according to claim 14, wherein the total length in the insertion direction is in a range of 400 to 600 micrometers.
16. The preparation for body surface application according to claim 15, wherein a sum of the lengths in the insertion direction of the sections 20 excluding the rearmost end section is 350 micrometers or less.
17. The preparation for body surface application according to any of claims 12 to 16, wherein the target substance comprises (i) one encapsulated in a microcapsule or (ii) fine particles having an average particle size of 10 micrometers or 25 less. 72
18. The preparation for body surface application according to any of claims 1 to 17, wherein the body surface comprises skin, cornea, oral soft tissue, gum, or nasal cavity mucous membrane.
19. The preparation for body surface application according to any of 5 claims 1 to 18, wherein the base is a high molecular weight substance.
20. The preparation for body surface application according to claim 19, wherein the high molecular weight substance is at least one kind selected from the group consisting of polysaccharides, proteins, polyvinyl alcohols, carboxy vinyl polymers, copolymers of these substances, and salts 10 of these substances.
21. The preparation for body surface application according to any of claims 1 to 20, wherein the target substance comprises peptides, proteins, nucleic acids, or polysaccharides.
22. The preparation for body surface application according to any of 15 claims 1 to 21, wherein the target substance comprises drugs, vaccines, nutrients, or components for cosmetics.
23. The preparation for body surface application according to any of claims 1 to 22, wherein the base includes a porous substance, and the target substance is held in the porous substance, so that the target substance is 20 sustainedly released.
24. A preparation for body surface application-holding sheet, in which one or two or more of the preparation for body surface application according to any of claims 1 to 23 are held on at least one surface of a sheet like support, wherein the preparation for body surface application can be 25 inserted into a body surface by pressing against the body surface. 73
25. The preparation for body surface application-holding sheet according to claim 24, wherein the preparation for body surface application includes an adhesive substance in the rearmost end section.
Applications Claiming Priority (7)
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JP2007302185 | 2007-11-21 | ||
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JP2008-182525 | 2008-07-14 | ||
JP2008182525 | 2008-07-14 | ||
PCT/JP2008/071224 WO2009066763A1 (en) | 2007-11-21 | 2008-11-21 | Preparation for application to body surface and preparation holding sheet for application to body surface |
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AU2008327083A1 true AU2008327083A1 (en) | 2009-05-28 |
AU2008327083B2 AU2008327083B2 (en) | 2014-01-16 |
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AU2008327083A Ceased AU2008327083B2 (en) | 2007-11-21 | 2008-11-21 | Preparation for application to body surface and preparation holding sheet for application to body surface |
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US (1) | US8491534B2 (en) |
EP (1) | EP2213284B1 (en) |
JP (1) | JP5538897B2 (en) |
KR (1) | KR101555391B1 (en) |
CN (1) | CN101868229A (en) |
AU (1) | AU2008327083B2 (en) |
CA (1) | CA2706404C (en) |
WO (1) | WO2009066763A1 (en) |
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KR101555391B1 (en) | 2015-09-23 |
CA2706404C (en) | 2017-04-11 |
EP2213284B1 (en) | 2017-11-15 |
KR20100098406A (en) | 2010-09-06 |
CN101868229A (en) | 2010-10-20 |
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US8491534B2 (en) | 2013-07-23 |
JP5538897B2 (en) | 2014-07-02 |
EP2213284A4 (en) | 2012-03-21 |
WO2009066763A1 (en) | 2009-05-28 |
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